RT 2 Profiler PCR Array Handbook

Transcription

1 December 2014 RT 2 Profiler PCR Array Handbook RT 2 Profiler PCR Array RT 2 First Strand Kit RT 2 SYBR Green qpcr Mastermix RT 2 SYBR Green Fluor qpcr Mastermix RT 2 SYBR Green ROX qpcr Mastermix RT 2 SYBR Green ROX FAST Mastermix For pathway-focused gene expression profiling using real-time RT-PCR Sample & Assay Technologies

2 QIAGEN Sample and Assay Technologies QIAGEN is the leading provider of innovative sample and assay technologies, enabling the isolation and detection of contents of any biological sample. Our advanced, high-quality products and services ensure success from sample to result. QIAGEN sets standards in: Purification of DNA, RNA, and proteins Nucleic acid and protein assays microrna research and RNAi Automation of sample and assay technologies Our mission is to enable you to achieve outstanding success and breakthroughs. For more information, visit

3 Contents Kit Contents 5 Shipping and Storage 11 Intended Use 12 Product Warranty and Satisfaction Guarantee 12 Technical Assistance 12 Safety Information 13 Quality Control 13 Introduction 14 First-strand cdna synthesis and mastermixes 14 Principle and procedure 15 RNA quality control using an RT 2 RNA QC PCR Array 20 Description of protocols 20 Equipment and Reagents to Be Supplied by User 21 Important Notes 22 Preparing a workspace free of DNA contamination 22 RNA preparation, quantification, and quality control 22 Recommended RNA preparation methods 22 RNA quantification and quality control 24 Genomic DNA contamination 25 Starting RNA amounts 26 Protocols cdna Synthesis Using the RT 2 First Strand Kit 27 Real-Time PCR for RT 2 Profiler PCR Arrays Formats A, C, D, E, F, G 29 Real-Time PCR for RT 2 Profiler PCR Arrays Format R 38 cdna Synthesis and Real-Time PCR for RT 2 Profiler PCR Arrays Format H 42 Troubleshooting Guide 48 Appendix A: Data Analysis Using the C T Method 50 Data analysis using the C T method for 96-well and 384-well formats 50 Data analysis using the C T method for Rotor-Disc formats 52 RT 2 Profiler PCR Array Handbook 12/2014 3

4 Detailed mathematical explanation of C T data analysis method 53 Appendix B: Protocol for Housekeeping Genes RT 2 Profiler PCR Arrays 55 References 57 Ordering Information 58 4 RT 2 Profiler PCR Array Handbook 12/2014

5 Kit Contents RT 2 Profiler PCR Array Format A* 96-well plate containing dried assays 2, 12, or 24 Optical Thin-Wall 8-Cap Strips (12 per 96-well plate) 24, 144, or 288 Handbook 1 * Suitable for use with the following real-time cyclers: Applied Biosystems models 5700, 7000, 7300, 7500, 7700, 7900HT, ViiA 7 (96-well block); Bio-Rad models icycler, iq 5, MyiQ, MyiQ2; Bio-Rad/MJ Research Chromo4 ; Eppendorf Mastercycler ep realplex models 2, 2S, 4, 4S; Stratagene models Mx3005P, Mx3000P ; Takara TP-800. RT 2 Profiler PCR Array Format C 96-well plate containing dried assays 2, 12, or 24 Optical Adhesive Film (1 per 96-well plate) 2, 12, or 24 Handbook 1 Suitable for use with the following real-time cyclers: Applied Biosystems models 7500 (Fast block), 7900HT (Fast block), StepOnePlus, ViiA 7 (Fast block). RT 2 Profiler PCR Array Format D 96-well plate containing dried assays 2, 12, or 24 Optical Thin-Wall 8-Cap Strips (12 per 96-well plate) 24, 144, or 288 Handbook 1 Suitable for use with the following real-time cyclers: Bio-Rad CFX96 ; Bio-Rad/MJ Research models DNA Engine Opticon, DNA Engine Opticon 2; Stratagene Mx4000. RT 2 Profiler PCR Array Handbook 12/2014 5

6 RT 2 Profiler PCR Array Format E 384 (4 x 96) option* 384-well plate containing dried assays 1 or 4 Optical Adhesive Film (1 per 384-well plate) 1 or 4 384EZLoad Covers (1 set of 4 per 384-well plate) 1 or 4 sets Handbook 1 * Suitable for use with the following real-time cyclers: Applied Biosystems models 7900HT (384-well block), ViiA 7 (384-well block); Bio-Rad CFX384. For a description of the 384 (4 x 96) option, see page 15. RT 2 Profiler PCR Array Format E 384 HT option 384-well plate containing dried assays 2, 12, or 24 Optical Adhesive Film (1 per 384-well plate) 2, 12, or 24 Handbook 1 Suitable for use with the following real-time cyclers: Applied Biosystems models 7900HT (384-well block), ViiA 7 (384-well block); Bio-Rad CFX384. For a description of the 384 HT option, see page 15. RT 2 Profiler PCR Array Format F 96-well plate containing dried assays 2, 12, or 24 Optical Adhesive Film (1 per 96-well plate) 2, 12, or 24 Handbook 1 Suitable for use with the following real-time cycler: Roche LightCycler 480 (96-well block). 6 RT 2 Profiler PCR Array Handbook 12/2014

7 RT 2 Profiler PCR Array Format G 384 (4 x 96) option * 384-well plate containing dried assays 1 or 4 Optical Adhesive Film (1 per 384-well plate) 1 or 4 384EZLoad Covers (1 set of 4 per 384-well plate) 1 or 4 sets Handbook 1 * Suitable for use with the following real-time cycler: Roche LightCycler 480 (384-well block). For a description of the 384 (4 x 96) option, see page 15. RT 2 Profiler PCR Array Format G 384 HT option 384-well plate containing dried assays 2, 12, or 24 Optical Adhesive Film (1 per 384-well plate) 2, 12, or 24 Handbook 1 Suitable for use with the following real-time cycler: Roche LightCycler 480 (384-well block). For a description of the 384 HT option, see page 15. RT 2 Profiler PCR Array Format H 96-well plate containing assays in solution; 96 x 96 chip compatible 1 Handbook 1 Suitable for use with the following real-time cycler: Fluidigm BioMark system. RT 2 Profiler PCR Array Format R** Rotor-Disc 100 containing dried assays 2, 12, or 24 Rotor-Disc Heat Sealing Film (1 per Rotor-Disc 100) 2, 12, or 24 Handbook 1 ** Suitable for use with the following real-time cyclers: QIAGEN Rotor-Gene Q; Rotor-Gene 6000; other Rotor-Gene cyclers. RT 2 Profiler PCR Array Handbook 12/2014 7

8 RT 2 First Strand Kit (12) Catalog no Number of 20 µl reactions 12 Buffer GE 24 µl 5x Buffer BC3 48 µl RE3 Reverse Transcriptase Mix 24 µl Control P2 12 µl RNase-Free Water 1 ml RT 2 SYBR Green qpcr Mastermix* (2) (12) (24) (8) (25 ml) Catalog no Number of array reactions 2x SYBR Green qpcr Mastermix, containing: HotStart DNA Taq Polymerase PCR Buffer dntp mix (datp, dctp, dgtp, dttp) SYBR Green dye 2 x 96-well 2 x 1.35 ml 12 x 96-well 12 x 1.35 ml 24 x 96-well 24 x 1.35 ml 4 x 384- well 8 x 1.35 ml 2000 x 25 µl reactions 25 ml * Suitable for use with real-time cyclers that do not require a reference dye, including: Bio-Rad models CFX96, CFX384; Bio-Rad/MJ Research models Chromo4, DNA Engine Opticon 2; Roche LightCycler 480 (96-well and 384-well). 8 RT 2 Profiler PCR Array Handbook 12/2014

9 RT 2 SYBR Green Fluor qpcr Mastermix* (2) (12) (24) (8) (25 ml) Catalog no Number of array reactions 2x SYBR Green Fluor qpcr Mastermix, containing: HotStart DNA Taq Polymerase PCR Buffer dntp mix (datp, dctp, dgtp, dttp) SYBR Green dye Fluorescein passive reference dye 2 x 96-well 2 x 1.35 ml 12 x 96-well 12 x 1.35 ml 24 x 96-well 24 x 1.35 ml 4 x 384- well 8 x 1.35 ml 2000 x 25 µl reactions 25 ml * Suitable for use with the following real-time cyclers: Bio-Rad models icycler, iq5, MyiQ, MyiQ2. RT 2 Profiler PCR Array Handbook 12/2014 9

10 RT 2 SYBR Green ROX qpcr Mastermix* (2) (12) (24) (8) (25 ml) Catalog no Number of array reactions 2x SYBR Green ROX qpcr Mastermix, containing: HotStart DNA Taq Polymerase PCR Buffer dntp mix (datp, dctp, dgtp, dttp) SYBR Green dye ROX passive reference dye 2 x 96-well 2 x 1.35 ml 12 x 96-well 12 x 1.35 ml 24 x 96-well 24 x 1.35 ml 4 x 384- well 8 x 1.35 ml 2000 x 25 µl reactions 25 ml * Suitable for use with the following real-time cyclers: Applied Biosystems models 5700, 7000, 7300, 7500 (Standard and Fast), 7700, 7900HT (Standard and Fast 96-well block, 384-well block), StepOnePlus, ViiA 7 (Standard and Fast 96-well block, 384-well block); Eppendorf Mastercycler ep realplex models 2, 2S, 4, 4S; Stratagene models Mx3000P, Mx3005P, Mx4000; Takara TP RT 2 Profiler PCR Array Handbook 12/2014

11 RT 2 SYBR Green ROX FAST Mastermix* (2) (12) (24) (8) (25 ml) Catalog no Number of array reactions 2x SYBR Green ROX FAST Mastermix, containing: HotStart DNA Taq Polymerase PCR Buffer dntp mix (datp, dctp, dgtp, dttp) SYBR Green dye ROX passive reference dye 2 x 96-well 2 x 1.35 ml 12 x 96-well 12 x 1.35 ml 24 x 96-well 24 x 1.35 ml 4 x 384- well 8 x 1.35 ml * Suitable for use with the Rotor-Gene Q (QIAGEN) and Rotor-Gene x 25 µl reactions 25 ml Note: RT 2 Profiler PCR Arrays cannot be used in the Cepheid SmartCycler or the Roche LightCycler 2.0. Shipping and Storage RT 2 Profiler PCR Array Formats A, C, D, E, F, G, and R are shipped at room temperature (15 25 C) or on ice or dry ice, depending on the destination and accompanying products. RT 2 Profiler PCR Array Format H is shipped on ice or dry ice. All RT 2 Profiler PCR Array Formats should be stored at 30 to 15 C upon arrival. When stored properly at 30 to 15 C, RT 2 Profiler PCR Arrays are stable for up to 1 year after delivery. RT² SYBR Green Mastermixes are shipped on cold packs. For long-term storage, keep tubes at 30 to 15 C. If the entire volume will not be used at once, we recommend dividing into aliquots and storing at 30 to 15 C. Avoid repeated freezing and thawing. If stored under these conditions, RT² SYBR Green Mastermixes are stable for 6 months after receipt. The RT² First Strand Kit is shipped frozen. For long-term storage, keep the kit at 30 to 15 C. If stored under these conditions, the RT² First Strand Kit is stable for 6 months after receipt. We recommend a maximum of 6 freeze-thaw cycles. RT 2 Profiler PCR Array Handbook 12/

12 Intended Use RT 2 Profiler PCR Arrays, the RT 2 First Strand Kit, the RT 2 Microfluidics qpcr Reagent System, and RT 2 SYBR Green Mastermixes are intended for molecular biology applications. These products are not intended for the diagnosis, prevention, or treatment of a disease. All due care and attention should be exercised in the handling of the products. We recommend all users of QIAGEN products to adhere to the NIH guidelines that have been developed for recombinant DNA experiments, or to other applicable guidelines. Product Warranty and Satisfaction Guarantee QIAGEN guarantees the performance of all products in the manner described in our product literature. The purchaser must determine the suitability of the product for its particular use. Should any product fail to perform satisfactorily due to any reason other than misuse, QIAGEN will replace it free of charge or refund the purchase price. We reserve the right to change, alter, or modify any product to enhance its performance and design. If a QIAGEN product does not meet your expectations, simply call your local Technical Service Department or distributor. We will credit your account or exchange the product as you wish. Separate conditions apply to QIAGEN scientific instruments, service products, and to products shipped on dry ice. Please inquire for more information. A copy of QIAGEN terms and conditions can be obtained on request, and is also provided on the back of our invoices. If you have questions about product specifications or performance, please call QIAGEN Technical Services or your local distributor (see back cover or visit Technical Assistance At QIAGEN, we pride ourselves on the quality and availability of our technical support. Our Technical Service Departments are staffed by experienced scientists with extensive practical and theoretical expertise in sample and assay technologies and the use of QIAGEN products. If you have any questions or experience any difficulties regarding RT 2 Profiler PCR Arrays, the RT 2 First Strand Kit, RT 2 SYBR Green Mastermixes, or QIAGEN products in general, please do not hesitate to contact us. QIAGEN customers are a major source of information regarding advanced or specialized uses of our products. This information is helpful to other scientists as well as to the researchers at QIAGEN. We therefore encourage you to contact us if you have any suggestions about product performance or new applications and techniques. 12 RT 2 Profiler PCR Array Handbook 12/2014

13 For technical assistance and more information, please see our Technical Support Center at or call one of the QIAGEN Technical Service Departments or local distributors (see back cover or visit Safety Information When working with chemicals, always wear a suitable lab coat, disposable gloves, and protective goggles. For more information, please consult the appropriate safety data sheets (SDSs). These are available online in convenient and compact PDF format at where you can find, view, and print the SDS for each QIAGEN kit and kit component. Quality Control In accordance with QIAGEN s Quality Management System, each lot of RT 2 Profiler PCR Arrays, RT 2 First Strand Kits, and RT 2 SYBR Green Mastermixes is tested against predetermined specifications to ensure consistent product quality. RT 2 Profiler PCR Array Handbook 12/

14 Introduction Real-time RT-PCR is a highly sensitive and reliable method for gene expression analysis. Its wide dynamic range makes real-time RT-PCR the preferred choice for the simultaneous quantification of both rare and abundant genes in the same sample. RT 2 Profiler PCR Arrays take advantage of the combination of real-time PCR performance and the ability of microarrays to detect the expression of many genes simultaneously. RT 2 Profiler PCR Arrays are designed to analyze a panel of genes related to a disease state or biological pathway. RT 2 Profiler PCR Arrays are especially suitable for researchers who are more familiar with or prefer real-time RT-PCR technology but are looking for the multigene profiling capabilities of a microarray. RT 2 Profiler PCR Arrays, RT 2 SYBR Green Mastermixes, and the RT 2 First Strand Kit have been optimized in combination for SYBR Green-based, real-time RT- PCR detection, providing the RT 2 Profiler PCR Arrays with superior sensitivity and wide linear dynamic ranges. The simplicity of the RT 2 Profiler PCR Arrays makes them accessible for routine use in every research laboratory. First-strand cdna synthesis and mastermixes Performance of RT² Profiler PCR Arrays is only guaranteed when used with RT² SYBR Green Mastermixes and the RT 2 First Strand Kit. Therefore, the use of the complete RT² Profiler PCR Array System is absolutely essential for obtaining accurate real-time PCR profiling results. The chemically modified and tightly controlled HotStart DNA Taq Polymerase enzyme and other proprietary chemical components in RT 2 SYBR Green Mastermixes uniquely provide more accurate SYBR Green results by preventing the amplification of primer dimers and other nonspecific products. They also help ensure high amplification efficiencies, even for genes that are difficult to amplify. When other sources of enzymes are tested with RT² Profiler PCR Arrays, primer dimers and other nonspecific products are frequently observed, leading to difficult-to-interpret SYBR Green-based, real-time PCR results. Real-time cyclers use different reference dyes to normalize their optics, therefore be sure to use the correct mastermix for the real-time cycler in your laboratory. The RT 2 First Strand Kit includes a proprietary buffer to eliminate any residual genomic DNA contamination in RNA samples before it can be amplified into secondary products that would otherwise cause false positive signals. The reverse-transcription controls (RTC) on the RT² Profiler PCR Array can only be evaluated with the built-in external RNA control of the RT 2 First Strand Kit. These controls do not yield results when used with other sources of reverse transcriptase or first strand synthesis kits. The buffer components and the magnesium concentration in the RT 2 First Strand Kit are also more compatible with RT² SYBR Green Mastermixes than other enzymes or kits, providing the RT² 14 RT 2 Profiler PCR Array Handbook 12/2014

15 Profiler PCR Arrays with maximum levels of sensitivity with nanogram to microgram amounts of total RNA. Principle and procedure RT 2 Profiler PCR Arrays are provided in 96-well plates, 96-well plates for use with 96 x 96 microfluidic chips, 384-well plates, or Rotor-Discs (Figures 1 4). RT 2 Profiler PCR Arrays in 96-well plates contain primer assays for 84 pathwayor disease-focused genes and 5 housekeeping genes. In addition, one well contains a genomic DNA control, 3 wells contain reverse-transcription controls, and 3 wells contain positive PCR controls (Figure 1). RT 2 Profiler PCR Arrays in 384-well plates are available in 384 (4 x 96) or 384 HT options. The 384 (4 x 96) option contains 4 replicate primer assays for each of 84 pathway- or disease-focused genes and 4 replicate primer assays for each of 5 housekeeping genes. In addition, 4 wells contain genomic DNA controls, 12 wells contain reverse-transcription controls, and 12 wells contain positive PCR controls (Figure 2). The 384 HT option contains primer assays for 370 pathway- or disease-focused genes and 5 housekeeping genes. In addition, 3 wells contain genomic DNA controls, 3 wells contain reverse-transcription controls, and 3 wells contain positive PCR controls (Figure 3). RT 2 Profiler PCR Arrays in Rotor-Disc 100 format contain primer assays for 84 pathway- or disease-focused genes and 5 housekeeping genes. In addition, one well contains a genomic DNA control, 3 wells contain reverse-transcription controls, and 3 wells contain a positive PCR control. Wells of the Rotor- Disc 100 do not contain assays (Figure 4). During the procedure, master mix is added to these wells for balance, but the wells are not used for analysis. RT 2 Profiler PCR Arrays in format H contain primer assays in solution to be aliquoted onto 96 x 96 chips. These include primer assays for 84 pathway- or disease-focused genes and 5 housekeeping genes. In addition, one well contains a genomic DNA control, 3 wells contain reverse-transcription controls, and 3 wells contain a positive PCR control (Figure 1). Custom RT 2 Profiler PCR Arrays contain primer assays defined by the customer. The plate layout and targeted genes are detailed in the Product Sheet provided. Each well of the RT 2 Profiler PCR Array (Formats A, C, D, E, F, G, R) contains a primer assay mixed with an inert dye (the dye is used for manufacturing quality control, and does not affect assay performance or fluorescence detection). Format H RT 2 Profiler PCR Arrays do not contain the dye. Definitions of controls in RT 2 Profiler PCR Arrays Assays for 5 housekeeping genes included in the arrays enable normalization of data. The genomic DNA control (GDC) is an assay that specifically detects RT 2 Profiler PCR Array Handbook 12/

16 nontranscribed genomic DNA contamination with a high level of sensitivity. The reverse-transcription control (RTC) is an assay that tests the efficiency of the reverse-transcription reaction performed with the RT 2 First Strand Kit by detecting template synthesized from the kit s built-in external RNA control. The positive PCR control (PPC) consists of a predispensed artificial DNA sequence and the assay that detects it. This control tests the efficiency of the polymerase chain reaction itself. Controls provided in replicates can be used to test for interwell, intra-plate consistency. Figure 1. RT 2 Profiler PCR Array Formats A, C, D, F, H layout. RT 2 Profiler PCR Array Formats A, C, D, F, H: Wells A1 to G12 each contain a real-time PCR assay for a pathway/disease/functionally related gene. Wells H1 to H5 contain a housekeeping gene panel to normalize array data (HK1 5). Well H6 contains a genomic DNA control (GDC). Wells H7 to H9 contain replicate reverse-transcription controls (RTC). Wells H10 to H12 contain replicate positive PCR controls (PPC). 16 RT 2 Profiler PCR Array Handbook 12/2014

17 Figure 2. RT 2 Profiler PCR Array Formats E, G 384 (4 x 96) option layout. RT 2 Profiler PCR Arrays with the 384 (4 x 96) option include 4 replicates of the same assays as provided in the 96-well format shown in Figure 1. Figure 3. RT 2 Profiler PCR Array Formats E, G 384 HT option layout. Wells A1 to P10 (1 370) each contain a real-time PCR assay for a pathway/disease/ functionally related gene. Wells P11 to P15 contain a housekeeping gene panel to normalize array data (HK1-5). Wells P16 to P18 contain replicate genomic DNA controls (GDC). Wells P19 to P21 contain replicate reverse-transcription controls (RTC). Wells P22 to P24 contain replicate positive PCR controls (PPC). RT 2 Profiler PCR Array Handbook 12/

18 Figure 4. RT 2 Profiler PCR Array Format R layout. Wells 1 to 84 each contain a real-time PCR assay for a pathway/disease/functionally related gene. Wells 85 to 89 contain a housekeeping gene panel to normalize array data. Well 90 contains a genomic DNA control. Wells 91 to 93 contain replicate reverse-transcription controls. Wells 94 to 96 contain replicate positive PCR controls. Wells 97 to 100 are empty. Workflow The procedure begins with the conversion of experimental RNA samples into first-strand cdna using the RT 2 First Strand Kit. Next, the cdna is mixed with an appropriate RT 2 SYBR Green Mastermix. This mixture is aliquoted into the wells of the RT 2 Profiler PCR Array. PCR is performed and finally relative expression is determined using data from the real-time cycler and the C T method. 18 RT 2 Profiler PCR Array Handbook 12/2014

19 RT 2 Profiler PCR Array Procedure Experimental samples Purify RNA Prepare cdna from purified RNA using RT 2 First Strand Kit Add cdna to RT 2 SYBR Green Mastermix Aliquot mix into RT 2 Profiler PCR Arrays Cycle in real-time cycler Analyze results RT 2 Profiler PCR Array Handbook 12/

20 RNA quality control using an RT 2 RNA QC PCR Array The RT 2 RNA QC PCR Array is designed to assess the quality of 12 RNA samples simultaneously before gene expression analysis using RT 2 Profiler PCR Arrays. Use of the RT 2 RNA QC PCR Array provides complete confidence in gene expression analysis results by enabling exclusion of substandard samples prior to analysis with RT 2 Profiler PCR Arrays. For further details, consult the RT 2 RNA QC PCR Array Handbook. Description of protocols This handbook contains 4 protocols. The first protocol details cdna synthesis by reverse transcription using purified RNA and the RT 2 First Strand Kit (page 27). This protocol should be performed prior to real-time PCR. The 3 additional protocols detail real-time PCR performed using the cdna prepared in the first protocol as the template. The protocol on page 29 should be used for 96-well and 384-well RT 2 Profiler PCR Arrays Formats A, C, D, E, F, G. The protocol on page 38 should be used for Rotor-Disc 100 RT 2 Profiler PCR Array Format R. For users of the Fluidigm BioMark real-time PCR system and RT 2 Profiler PCR Array Formats H, the protocol on page 42 should be used for cdna synthesis, preamplification, and real-time PCR. 20 RT 2 Profiler PCR Array Handbook 12/2014

21 Equipment and Reagents to Be Supplied by User When working with chemicals, always wear a suitable lab coat, disposable gloves, and protective goggles. For more information, consult the appropriate material safety data sheets (MSDSs), available from the product supplier. In addition to the RT 2 Profiler PCR Array, RT 2 First Strand Kit, and RT 2 SYBR Green Mastermix, the following are required: Purified RNA samples Real-time PCR cycler High-quality, nuclease-free water. Do not use DEPC-treated water. Multichannel pipettor Single-channel pipettor (if using RT 2 PreAMP Pathway Primer Mix) Nuclease-free pipet tips and tubes Optional: XpressRef Universal Total RNA to control PCR conditions is available for human (cat. no ), mouse (cat. no ), and rat (cat. no ) Optional: RT 2 PCR Array Loading Reservoir (cat. no ) For users of RT 2 Profiler PCR Array format H with the Fluidigm BioMark system 20x DNA Binding Dye Sample Loading Reagent (Fluidigm, cat. no ) 8-strip PCR tubes Low EDTA TE buffer (0.1 mm EDTA) RT 2 Profiler PCR Array Handbook 12/

22 Important Notes Preparing a workspace free of DNA contamination For accurate and reproducible PCR Array results, it is important to avoid contamination of the assay with foreign DNA. Any DNA contamination will artificially inflate the SYBR Green signal, yielding skewed gene expression profiles and false-positive signals. The most common sources of DNA contamination are the products of previous experiments spread into the air of the working environment. To set up and maintain a working environment free of DNA contamination, follow the guidelines below. Wear gloves throughout the procedure. Use only fresh PCR-grade reagents (water) and labware (tips and tubes). Physically separate the workspaces used for PCR setup and post-pcr processing or non-pcr operations. Decontaminate the PCR workspace and labware (pipettor barrels, tube racks, etc.) before each use with UV light (to render any contaminating DNA ineffective in PCR through the formation of thymidine dimers) or with 10% bleach (to chemically inactivate and degrade any DNA). Close all tubes containing PCR products once you are finished adding or removing volumes. Before discarding any labware (tips or tubes) containing PCR products or other DNA, treat with 10% bleach. Do not remove the RT 2 Profiler PCR Array from its protective, sealed bag until immediately before use. Do not leave labware (tubes and tip boxes) exposed to the air for long periods of time. Do not open any previously run and stored RT 2 Profiler PCR Array. Removing the thin-wall, 8-cap strips or the adhesive film from PCR arrays releases PCR product DNA into the air where it may affect the results of future real-time PCR experiments. RNA preparation, quantification, and quality control High-quality RNA is essential for obtaining good, real-time PCR results. The most important prerequisite for any gene expression analysis experiment is consistently high-quality RNA from every experimental sample. Residual traces of proteins, salts, or other contaminants may degrade the RNA or decrease the efficiency of enzyme activities necessary for optimal reverse transcription and real-time PCR performance. Recommended RNA preparation methods High quality total RNA for your real-time PCR experiment should be prepared using one of the methods described below, depending on the biological 22 RT 2 Profiler PCR Array Handbook 12/2014

23 sample. For optimal results, RNA samples should be suspended in RNase-free water. Do not use DEPC-treated water. Cultured cells We recommend the mirneasy Mini Kit (cat. no )* for RNA purification from cultured cells. It is important to perform the on-column DNase digestion step described in the mirneasy Mini Handbook (using the RNase-Free DNase Set [cat. no ]). Tissue samples We recommend the RNeasy Microarray Tissue Mini Kit (cat. no ) including the optional on-column DNase digestion step described in the RNeasy Microarray Tissue Handbook (using the RNase-Free DNase Set [cat. no ]). Formalin-fixed paraffin-embedded (FFPE) samples We recommend the mirneasy FFPE Kit (cat. no ) for RNA purification from FFPE samples. Small samples yielding <100 ng total RNA We recommend the mirneasy Micro Kit (cat. no ) for RNA purification from small samples. Whole blood samples We recommend the PAXgene Blood RNA Kit (cat. no ) for preparation of total RNA from whole blood samples. Alternatively, the QIAamp RNA Blood Mini Kit (cat. no ) can also be used for this purpose. Total RNA isolated using a phenol-based method Total RNA from any biological source material prepared using a phenol-based method (e.g., QIAzol Lysis Reagent, TRIzol Reagent, RNAzol Reagent) should be further purified using the mirneasy Mini Kit. It is important to perform the on-column DNase digestion step described in the mirneasy Mini Handbook. Other biological samples Refer to the existing literature to find protocols for high-quality RNA purification from other biological samples or contact QIAGEN Technical Service. * mirneasy kits yield total RNA as well as mirna isolation. If no microrna analysis is planned, the corresponding RNeasy kits may be substituted for the listed mirneasy kits. RT 2 Profiler PCR Array Handbook 12/

24 RNA quantification and quality control For best results from the RT 2 Profiler PCR Array, all RNA samples should also demonstrate consistent quality according to the criteria described below. In addition, as some contaminants are difficult to detect by simply looking at RNA integrity and can be missed by UV spectrophotometry, it is essential to choose an appropriate RNA purification method for your biological sample as described on page Concentration and purity determined by UV spectrophotometry The concentration and purity of RNA should be determined by measuring the absorbance in a spectrophotometer. Prepare dilutions and measure absorbance in RNase-free water. The spectral properties of nucleic acids are highly dependent on ph. An absorbance reading of 1.0 at 260 nm in a 1 cm detection path corresponds to an RNA concentration of 40 µg/ml. A 260 :A 230 ratio should be greater than 1.7 A 260 :A 280 ratio should be 1.8 to 2.0 Concentration determined by A 260 should be >40 µg/ml Ribosomal RNA band integrity Run an aliquot of each RNA sample on a denaturing agarose gel or the Agilent Bioanalyzer using an RNA 6000 Nano LabChip. Verify that there are sharp bands/peaks present for both the 18S and 28S ribosomal RNAs (Figure 5). Any smearing of the RNA bands or shoulders on the RNA peaks indicates that degradation has occurred in the RNA sample. For reliable data from RT 2 Profiler PCR Arrays, an RNA Integrity Number (RIN) of 7 or higher is recommended. Consistent RIN values across multiple samples within each experiment are desirable for reliable quality data comparisons. Samples with degraded RNA, such as from FFPE blocks/slides, with RINs less than 7, may be of sufficient quality, but the final PCR data must be checked for quality. 24 RT 2 Profiler PCR Array Handbook 12/2014

25 A B Figure 5. Ribosomal RNA integrity. A Agilent Bioanalyzer electropherogram of high-quality total RNA showing sharp peaks for the 18S (left) and 28S (right) ribosomal RNA. Due to high quality of the RNA, peaks do not have shoulders (especially to the left of each peak). B Agarose gel electrophoresis shows sharp bands (especially at the bottom of each band) for 28S and 18S ribosomal RNA. RT 2 RNA QC PCR Array (optional) The RT 2 RNA QC PCR Array is particularly useful for researchers who are unsure of their RNA purification technique. The RT 2 RNA QC PCR Array and the RT 2 First Strand Kit (sold separately) test for a number of RNA quality control parameters including: High and low housekeeping gene expression levels Reverse transcription and polymerase chain reaction efficiency Genomic and general DNA contamination For further details, consult the RT 2 RNA QC PCR Array Handbook. Genomic DNA contamination Eliminating genomic DNA contamination is essential for obtaining optimal realtime gene expression profiling results using the RT 2 Profiler PCR Array. The genomic DNA control in each RT 2 Profiler PCR Array specifically tests for genomic DNA contamination in each sample during each run. A genomic DNA control threshold cycle value of less than 35 indicates the presence of a detectable amount of genomic DNA contamination that should be addressed. To remove any residual contamination from your RNA samples, we strongly recommend RNA purification using the RNeasy Mini Kit including the optional on-column DNase digestion step, followed by cdna synthesis using the RT 2 First Strand Kit. If required, individual, species-specific RT 2 qpcr Primer gdna Controls are available. RT 2 Profiler PCR Array Handbook 12/

26 Starting RNA amounts The RT 2 Profiler PCR Array System provides results with as little as 25 ng or as much as 5 µg total RNA per array.* For smaller starting RNA amounts, the RT 2 PreAMP cdna Synthesis Kit and RT 2 PreAMP Pathway Primer Mix enable gene expression analysis from as little as 1 ng total RNA or 100 ng RNA from FFPE samples by preamplifying first strand cdna. This allows gene expression analysis from samples such as fine needle biopsy samples, laser captured microdissection samples, stem cell clusters or embryoid bodies, FACS generated cells, or FFPE samples. For more details, see the RT 2 PreAMP cdna Synthesis Handbook. The optimal amount of starting material depends on the relative abundance of the transcripts of interest. Lower abundance transcripts require more RNA; higher abundance transcripts require less RNA. Greater amounts of input total RNA yield a greater number of positive calls (i.e., genes expressed in the linear dynamic range of the method). Lower amounts of input total RNA yield a smaller number of positive calls and increase false negative calls. For successful results and maximum positive call rates, we recommend that firsttime users start with 0.5 µg total RNA for 96-well plate formats, 0.8 µg total RNA for Rotor-Disc 100 formats, 400 ng total RNA for format E and G 384 (4 x 96) option, or 1 µg total RNA for format E and G 384 HT option. It is important to use a consistent amount of total RNA for all samples in a single experiment. * Using more RNA than the recommended maximum may potentially overload the restriction enzyme system. 26 RT 2 Profiler PCR Array Handbook 12/2014

27 Protocol: cdna Synthesis Using the RT 2 First Strand Kit Use of the RT 2 First Strand Kit is critical for obtaining optimal results and for detection of the reverse transcription controls contained in the RT 2 Profiler PCR Array. If using the Fluidigm BioMark real-time PCR system, refer to page 42 for the cdna synthesis protocol and for sample/plate preparation instructions. Important points before starting Use the same amount of total RNA for reverse transcription of each sample. First-time users are recommended to start with 0.5 µg total RNA for 96-well plate formats, 0.8 µg total RNA for Rotor-Disc 100 formats, 400 ng total RNA for format E and G 384 (4 x 96) option, or 1 µg total RNA for format E and G 384 HT option. Use of less than 100 ng RNA will result in a high rate of false negatives. If 100 ng RNA is available, refer to the RT 2 PreAMP cdna Synthesis Handbook. Use of more than the recommended amount of RNA may potentially overload the system. Do not use DEPC-treated water. Use high-quality, nuclease-free water. The RT 2 First Stand Kit is not compatible with the chemicals in DNA-free kits from Ambion. If your RNA sample has been treated with DNA-free reagents, contact QIAGEN Technical Service. Procedure 1. Thaw the reagents of the RT 2 First Strand Kit. Briefly centrifuge (10 15 s) to bring the contents to the bottom of the tubes. 2. Prepare the genomic DNA elimination mix for each RNA sample according to Table 1. Mix gently by pipetting up and down and then centrifuge briefly. Table 1. Genomic DNA elimination mix Component Amount RNA* 25 ng 5 µg Buffer GE 2 µl RNase-free water Variable Total volume 10 µl * If using the kit for the first time, use the RNA amount recommended in Important points before starting above. RT 2 Profiler PCR Array Handbook 12/

28 3. Incubate the genomic DNA elimination mix for 5 min at 42 C, then place immediately on ice for at least 1 min. 4. Prepare the reverse-transcription mix according to Table 2. Table 2. Reverse-transcription mix Component Volume for 1 reaction Volume for 2 reactions Volume for 4 reactions 5x Buffer BC3 4 µl 8 µl 16 µl Control P2 1 µl 2 µl 4 µl RE3 Reverse Transcriptase Mix 2 µl 4 µl 8 µl RNase-free water 3 µl 6 µl 12 µl Total volume 10 µl 20 µl 40 µl 5. Add 10 µl reverse-transcription mix to each tube containing 10 µl genomic DNA elimination mix. Mix gently by pipetting up and down. 6. Incubate at 42 C for exactly 15 min. Then immediately stop the reaction by incubating at 95 C for 5 min. 7. Add 91 µl RNase-free water to each reaction. Mix by pipetting up and down several times. 8. Place the reactions on ice and proceed with the real-time PCR protocol. If you wish to store the reactions prior to real-time PCR, transfer them to a 15 to 30 C freezer. For quality control analysis using the RT 2 RNA QC PCR Array, follow the protocol in the RT 2 RNA QC PCR Array Handbook using a 6 µl aliquot of the diluted cdna template. 28 RT 2 Profiler PCR Array Handbook 12/2014

29 Protocol: Real-Time PCR for RT 2 Profiler PCR Arrays Formats A, C, D, E, F, G This protocol describes real-time PCR using RT 2 Profiler PCR Arrays in combination with RT 2 SYBR Green Mastermixes. Use of RT 2 SYBR Green Mastermixes is critical to obtain accurate results from the RT 2 Profiler PCR Array. If unsure of the RNA quality or purification technique, examine the RNA quality before performing this protocol using species- and cycler-specific RT 2 RNA QC PCR Arrays. For RT 2 Profiler PCR Array Format H, refer to the protocol on page 42. Important points before starting Ensure that the RT 2 SYBR Green Mastermix and the RT 2 Profiler PCR Array format are suitable for your real-time cycler (see page 5). The format of the RT 2 Profiler PCR Array is indicated by the last letter of the catalog number. An incorrect RT 2 Profiler PCR Array format will not fit the real-time cycler properly and may damage the real-time cycler. Do not cut the plastic plate of the RT 2 Profiler PCR Array. For accuracy and precision, ensure that micropipettors are calibrated before beginning the protocol. Be sure not to introduce bubbles into the wells of the RT 2 Profiler PCR Array when pipetting. Do not use DEPC-treated water. Use high-quality, nuclease-free water. If precipitates are present in the Mastermix tubes, warm the reagents at 42 C for 1 min and vortex briefly to dissolve. Repeat if necessary. Procedure 1. Briefly centrifuge the RT 2 SYBR Green Mastermix (10 15 s) to bring the contents to the bottom of the tube. Note: As the RT 2 SYBR Green Mastermix contains HotStart DNA Taq Polymerase that is active only after heat activation, reactions can be prepared at room temperature (15 25 C). 2. Prepare the PCR components mix in a 5 ml tube or a loading reservoir depending on the RT 2 Profiler PCR Array format, as described in Table 3. RT 2 Profiler PCR Array Handbook 12/

30 Table 3. PCR components mix Array format: 2x RT 2 SYBR Green Mastermix 96-well A, C, D, F 384 (4 x 96) option E, G 384 HT option E, G 1350 µl 650 µl 2100 µl cdna synthesis reaction 102 µl 102 µl 102 µl RNase-free water 1248 µl 548 µl 1998 µl Total volume 2700 µl 1300 µl 4200 µl Note: This provides an excess volume of 300 µl (formats A, C, D, F), 340 µl (formats E, G: 384 (4 x 96) option), or 360 µl (formats E, G: 384 HT option) to allow for pipetting errors. Perform pipetting steps as precisely as possible to ensure that each well receives the required volume. Note: For Custom RT 2 Profiler PCR Arrays, prepare a volume of PCR components mix 10% greater than required for the total number of reactions to be performed. Note: Save the remaining 9 µl cdna synthesis reaction at 15 to 30 C, as it may be needed to perform quality control analysis. 3. Dispense the PCR components mix into the RT 2 Profiler PCR Array depending on the RT 2 Profiler PCR Array format, as described below. Note: Change pipet tips following each pipetting step to avoid crosscontamination between the wells. Note: If using an instrument to automate this step, contact Technical Service for plate specifications. Formats A, C, D, or F (96-well) Carefully remove the RT 2 Profiler PCR Array from its sealed bag. Optional: If the PCR components mix is in a tube, transfer to a loading reservoir, such as the RT 2 PCR Array Loading Reservoir (cat. no ). Add 25 µl PCR components mix to each well of the RT 2 Profiler PCR Array using an 8-channel pipettor, or a 12-channel pipettor using only 8 tips. Proceed to step RT 2 Profiler PCR Array Handbook 12/2014

31 Formats E or G 384 (4 x 96) option Note: Each 384-well plate contains 4 replicates of 96 assays that can be used for analysis of 4 samples, with reactions for each sample separated from one another by only one well. The spacing between the tips of standard multichannel pipettors allows rows or columns to be skipped when adding each sample. Be sure to load each sample into the correct set of wells using Figure 6 as a guide. Carefully remove the RT 2 Profiler PCR Array from its sealed bag. Optional: If the PCR components mix is in a tube, transfer to a loading reservoir, such as the RT 2 PCR Array Loading Reservoir (cat. no ). Add PCR components mix to each well of the RT 2 Profiler PCR Array using an 8-channel pipettor, or a 12-channel pipettor using only 8 tips, and the 384EZLoad Covers (provided) using Figure 6 as a guide. Place 384EZLoad Cover 1 (white) on the plate. Add 10 µl PCR components mix for sample 1 to the open wells (odd number wells of rows A, C, E, G, I, K, M, and O). Remove and discard 384EZLoad Cover 1. Place 384EZLoad Cover 2 (yellow) on the plate. Add 10 µl PCR components mix for sample 2 to the open wells (even number wells of rows A, C, E, G, I, K, M, and O). Remove and discard 384EZLoad Cover 2. Place 384EZLoad Cover 3 (black) on the plate. Add 10 µl PCR components mix for sample 3 to the open wells (odd number wells of rows B, D, F, H, J, L, N, and P). Remove and discard 384EZLoad Cover 3. Place 384EZLoad Cover 4 (red) on the plate. Add 10 µl PCR components mix for sample 4 to the open wells (even number wells of rows B, D, F, H, J, L, N, and P). Remove and discard 384EZLoad Cover 4. RT 2 Profiler PCR Array Handbook 12/

32 Sample A B C D E F G H I J K L M N O P Sample A B C D E F G H I J K L M N O P Sample A B C D E F G H I J K L M N O P RT 2 Profiler PCR Array Handbook 12/2014

33 Sample A B C D E F G H I J K L M N O P Figure 6. Loading RT 2 Profiler PCR Arrays Formats E or G 384 (4 x 96) option. Add 10 µl PCR components mix for each of 4 samples into the staggered wells with the same number as indicated in the figure. Proceed to step 4. Formats E or G 384 HT option Carefully remove the RT 2 Profiler PCR Array from its sealed bag. Optional: If the PCR components mix is in a tube, transfer to a loading reservoir, such as the RT 2 PCR Array Loading Reservoir (cat. no ). Add 10 µl PCR components mix to each well of the RT 2 Profiler PCR Array using an 8-channel pipettor, or a 12-channel pipettor using only 8 tips. Proceed to step 4. Custom RT 2 Profiler PCR Arrays Carefully remove the RT 2 Profiler PCR Array from its sealed bag. Optional: If the PCR components mix is in a tube, transfer to a loading reservoir, such as the RT 2 PCR Array Loading Reservoir (cat. no ). Add PCR components mix to each well of the RT 2 Profiler PCR Array: 25 µl per well for 96-well Custom RT 2 Profiler PCR Arrays or 10 µl per well for 384-well Custom RT 2 Profiler PCR Arrays. Proceed to step Carefully, tightly seal the RT 2 Profiler PCR Array with Optical Thin- Wall 8-Cap Strips (Formats A and D) or Optical Adhesive Film (Formats C, E, F, and G). IMPORTANT: Users of Bio-Rad and Eppendorf real-time cyclers must ensure that the real-time cycler has been calibrated to use clear, flat optical caps with RT 2 Profiler PCR Array plates prior to initiating the run. RT 2 Profiler PCR Array Handbook 12/

34 5. Centrifuge for 1 min at 1000 g at room temperature (15 25 C) to remove bubbles. Visually inspect the plate from underneath to ensure no bubbles are present in the wells. Note: The presence of bubbles in the wells interferes with results. 6. Place the RT 2 Profiler PCR Array on ice while setting up the PCR cycling program. Note: The RT 2 Profiler PCR Array containing PCR components mix may be stored at 15 to 30 C wrapped in aluminum foil for up to one week if desired. 7. Program the real-time cycler according to Table 4, 5, or 6, depending on the real-time cycler used. If prompted by your cycler software, select Absolute Quantitation to begin. Note: For additional help with instrument setup, see our Instrument-Specific Setup Instructions and Protocol Files at Table 4. Cycling conditions* for Applied Biosystems, Bio-Rad, Stratagene, and Eppendorf cyclers Cycles Duration Temperature Comments 1 10 min 95 C HotStart DNA Taq Polymerase is activated by this heating step s 95 C 1 min 60 C Perform fluorescence data collection. * Recommended for the following cyclers: Applied Biosystems models 5700, 7000, 7300, 7500, 7700, 7900HT, StepOnePlus,; Bio-Rad models icycler, iq5, MyiQ, MyiQ2, CFX96, CFX384; Stratagene models Mx3000P, Mx3005P, Mx4000P; Eppendorf Mastercycler ep realplex models 2, 2S, 4, 4S. For Bio-Rad models CFX96 and CFX384 and ABI ViiA 7: adjust the ramp rate to 1 C/s. For Eppendorf Mastercyler ep realplex models 2, 2S, 4, and 4S: for the Silver Thermoblock, adjust the ramp rate to 26%; for the Aluminum Thermoblock, adjust the ramp rate to 35%. Refer to the Instrument Setup Guide at for detailed setup instructions. 34 RT 2 Profiler PCR Array Handbook 12/2014

35 Table 5. Cycling conditions for Roche LightCycler 480* Cycles Duration Temperature Comments 1 10 min 95 C HotStart DNA Taq Polymerase is activated by this heating step s 95 C 1 min 60 C Perform fluorescence data collection. * Recommended for the Roche LightCycler 480. If using a Roche LightCycler 480, adjust the ramp rate to 1.5 C/s. Refer to the Instrument Setup Guide at for more information on other required changes to settings for Melt Curve Acquisition. Table 6. Cycling conditions for Bio-Rad and Takara cyclers and all other cyclers Cycles Duration Temperature Comments 1 10 min 95 C HotStart DNA Taq Polymerase is activated by this heating step s 95 C s 55 C Perform fluorescence data collection. Different cyclers need different lengths of time to detect the fluorescent signal. Choose the appropriate time for the annealing step (55 C) for your cycler. 30 s 72 C Recommended for the following cyclers: Bio-Rad/MJ Research models Chromo4, DNA Engine Opticon, DNA Engine Opticon 2; Takara TP-800; all other cyclers. 8. Place the RT 2 Profiler PCR Array in the real-time cycler. If recommended by the cycler user manual, use a compression pad with RT 2 Profiler PCR Arrays sealed with optical adhesive film (formats C, E, F, and G). Start the run. 9. Calculate the threshold cycle (C T ) for each well using the real-time cycler software, as described in the following steps. Note: If using the Roche LightCycler 480, there are 2 options for data analysis: using the second derivate max setting (in this case there is no need to calculate the C T ) or using Fit Points (in this case the C T should be defined manually as described in step 11). RT 2 Profiler PCR Array Handbook 12/

36 10. Define the baseline by choosing the automated baseline option if the cycler has the adaptive baseline function. If the cycler does not have the adaptive baseline function, set the baseline manually. To set the baseline manually, use the linear view of the amplification plots to determine the earliest visible amplification. Set the cycler to use the readings from cycle number 2 through 2 cycles before the earliest visible amplification, but no more than cycle 15. The earliest amplification will usually be visible between cycles 14 and Manually define the threshold by using the log view of the amplification plots. Choose a threshold value above the background signal but within the lower one-third to lower one-half of the linear phase of the amplification plot. Note: Ensure that the threshold values are the same across all RT 2 Profiler PCR Array runs in the same analysis. The absolute position of the threshold is less critical than its consistent position across arrays. If the RNA sample is of sufficient quality, the cycling program has been carried out correctly, and threshold values have been defined correctly, the value of C T PPC should be 20 ± 2 for all arrays or samples. 12. Export the C T values for all wells to a blank Excel spreadsheet for use with the SABiosciences PCR Array Data Analysis Template Excel or Web-based software. Note: Excel-based PCR Array Data Analysis Templates for 96-well, 384- well, and custom formats are available at Web-based PCR Array Data Analysis Software is available at Recommended: Perform dissociation (melting) curve analysis to verify PCR specificity. Run a melting curve program and generate a first derivative dissociation curve for each well using the real-time cycler software. A single peak should appear in each reaction at temperatures greater than 80 C. Note: If your instrument does not have a default melting curve program, run the following program instead: 95 C, 1 min; 65 C, 2 min (optics off); 65 C to 95 C at 2 C/min (optics on). Note: For cycler-specific melting curve analysis settings, please refer to the Instrument Setup Guide for your cycler at Note: Plates can be stored at 15 to 30 C wrapped in aluminum foil and melting curve analysis performed at a later time. When ready to perform melting curve analysis, warm the plate to room temperature (15 25 C), place it in the real-time cycler, and run the melting curve analysis program. 36 RT 2 Profiler PCR Array Handbook 12/2014

37 Note: Visually inspect the plate after the run for any signs of evaporation from any of the wells. If evaporation is observed, note which wells are affected, as this may affect the results of data analysis. Note: Do not open any previously processed RT 2 Profiler PCR Array. Removing the Optical Thin-Wall 8-Cap Strips or the Optical Adhesive Film from RT 2 Profiler PCR Arrays releases PCR product into the air where it may contaminate and affect the results of future real-time PCR experiments. RT 2 Profiler PCR Array Handbook 12/

38 Protocol: Real-Time PCR for RT 2 Profiler PCR Arrays Format R Important points before starting Ensure that RT 2 Profiler PCR Array Format R and RT 2 SYBR Green ROX FAST Mastermix are used with a Rotor-Gene cycler. The format of the RT 2 Profiler PCR Array is indicated by the last letter of the catalog number. For accuracy and precision, ensure that micropipettors are calibrated before beginning the protocol. Be sure not to introduce bubbles into the wells of the RT 2 Profiler PCR Array when pipetting. Do not use DEPC-treated water. Use high-quality, nuclease-free water. If precipitates are present in the Mastermix tubes, warm the reagents at 42 C for 1 min and vortex briefly to dissolve. Repeat if necessary. Procedure 1. Briefly centrifuge the RT 2 SYBR Green ROX FAST Mastermix, water, and cdna synthesis reaction (10 15 s) to bring the contents to the bottom of the tubes. Note: As the RT 2 SYBR Green ROX FAST Mastermix contains HotStart DNA Taq Polymerase that is active only after heat activation, reactions can be prepared at room temperature (15 25 C). 2. Prepare the PCR components mix in a 5 ml tube, as described in Table 7. Table 7. PCR components mix Array format: Rotor-Disc 100 2x RT 2 SYBR Green ROX FAST Mastermix 1150 µl cdna synthesis reaction 102 µl RNase-free water 1048 µl Total volume 2300 µl Note: This provides an excess volume of 300 µl to allow for pipetting errors. Perform pipetting steps as precisely as possible to ensure that each well receives the correct volume. 38 RT 2 Profiler PCR Array Handbook 12/2014

39 Note: Save the remaining 9 µl cdna synthesis reaction at 15 to 30 C, as it may be needed to perform quality control analysis using the RT 2 RNA QC PCR Array. 3. Carefully remove the RT 2 Profiler PCR Array from its sealed bag. Slide the array into the Rotor-Disc 100 Loading Block using the tab at position A1 and the tube guide holes. 4. Add 20 µl PCR components mix to each well of the RT 2 Profiler PCR Array. Proceed to step 5. Note: Change pipet tips following each pipetting step to avoid crosscontamination between the wells. Note: PCR components mix can be dispensed manually or using the QIAgility ( Note: Although wells do not contain assays, it is essential to add PCR components mix for optimized balancing of the RT 2 Profiler PCR Array. 5. Carefully seal the RT 2 Profiler PCR Array with Rotor-Disc Heat- Sealing Film using the Rotor-Disc Heat Sealer. For detailed instructions, see the Rotor-Gene Q User Manual. Note: The RT 2 Profiler PCR Array containing PCR components mix may be stored at 15 to 30 C wrapped in aluminum foil for up to one week if desired. 6. Program the real-time cycler according to Table 8. Note: For additional help with instrument setup, see our Instrument-Specific Setup Instructions and Protocol Files at: Table 8. Cycling conditions for Rotor-Gene cyclers Cycles Duration Temperature Comments 1 10 min 95 C HotStart DNA Taq Polymerase is activated by this heating step s 95 C 30 s 60 C Perform fluorescence data collection. 7. Insert the RT 2 Profiler PCR Array into the Rotor-Disc 100 Rotor and secure with the Rotor-Disc 100 Locking Ring. Start the run. For detailed instructions, see the Rotor-Gene Q User Manual. 8. Calculate the threshold cycle (C T ) for each well using the real-time cycler software. To define the baseline, select Dynamic Tube RT 2 Profiler PCR Array Handbook 12/

40 (default analysis setting) to ensure the average background of each well is determined just before amplification commences. Optional: Select Ignore First. Fluorescent signal from the initial cycles may not be representative of the remainder of the run. Thus, better results may be achieved if the initial cycles are ignored. Up to 5 cycles can be ignored. Optional: Select Noise Slope Correction. Selection of this option can improve data whose baseline (initial cycles) is noticeably sloped. Noise Slope Correction improves the data when raw data backgrounds are observed to slope upward or downward before the takeoff point (C T ). Note: Ensure that the settings are the same across all RT 2 Profiler PCR Array runs in the same analysis. 9. Manually define the threshold by using the log view of the amplification plots. Choose a threshold value above the background signal. The threshold value should be in the lower half of the linear phase of the amplification plot. Note: Ensure that the threshold values are the same across all RT 2 Profiler PCR Array runs in the same analysis. The absolute position of the threshold is less critical than its consistent position across arrays. If the RNA sample is of sufficient quality, the cycling program has been carried out correctly, and threshold values have been defined correctly, the value of C T PPC should be 14 ± 2 for all arrays or samples. 10. Export the C T values for all wells to a blank Excel spreadsheet for use with the PCR Array Data Analysis Template Excel or Web-based software. Note: Excel-based PCR Array Data Analysis Templates for the RT 2 Profiler PCR Array Rotor-Gene format are available at Web-based PCR Array Data Analysis Software is available at Recommended: Perform dissociation (melting) curve analysis to verify PCR specificity. Run a melting curve program and generate a first derivative dissociation curve for each well using the real-time cycler software. A single peak should appear in each reaction. Note: Melting curve analysis can be added during creation of the Rotor- Gene Q PCR program. Note: For Rotor-Gene Q melting curve analysis settings, refer to the Instrument Setup Guide at Note: Rotor-Discs can be stored at 15 to 30 C wrapped in aluminum foil and melting curve analysis performed at a later time. When ready to 40 RT 2 Profiler PCR Array Handbook 12/2014

41 perform melting curve analysis, warm the plate to room temperature (15 25 C), place it in the real-time cycler, and run the melting curve analysis program. Note: Visually inspect the Rotor-Disc after the run for any signs of evaporation from any of the wells. If evaporation is observed, note which wells are affected, as this may affect the results of data analysis. Note: Do not open any previously processed RT 2 Profiler PCR Array. Removing the film from RT 2 Profiler PCR Arrays releases PCR product into the air where it may contaminate and affect the results of future real-time PCR experiments. RT 2 Profiler PCR Array Handbook 12/

42 Protocol: cdna Synthesis and Real-Time PCR for RT 2 Profiler PCR Arrays Format H This protocol is for users of the Fluidigm BioMark HD System. In this protocol, cdna synthesis is performed using the RT² Microfluidics qpcr Reagent System. Next, preamplification is performed using the RT 2 PreAMP Pathway Primer Mix Format H. Finally, real-time PCR is performed using RT 2 Profiler PCR Array Format H in combination with Microfluidics qpcr Master Mix (contains EvaGreen ). Considerations of RNA amount to be used The RT² Microfluidics qpcr System yields results with as little as 10 ng or as much as 1 µg total RNA per well reaction. However, the optimal amount of starting material depends on the relative abundance of the transcripts of interest. Lower abundance transcripts require more RNA; higher abundance transcripts require less RNA. Greater amounts of input RNA yield greater number of positive calls; that is, genes expressed in the linear dynamic range of the method. Important: Use a consistent amount of total RNA for all samples in a single experiment to be characterized and compared. Procedure cdna synthesis using the RT² Microfluidics qpcr Reagent System 1. Thaw Buffer GE2 and BC4 Solution (RT master mix). Mix each solution by flicking the tubes. Centrifuge briefly to collect residual liquid from the sides of the tubes and then store on ice. 2. Prepare the genomic DNA elimination mix for each RNA sample in one well of a 96-well plate according to Table 9. Table 9. Genomic DNA elimination mix Component RNA Amount for each well 10 ng 1 µg* Buffer GE2 6 µl RNase-free water Variable Total volume 14 µl * If performing the experiment for the first time, we recommend 1 µg RNA. 42 RT 2 Profiler PCR Array Handbook 12/2014

43 3. Incubate the genomic DNA elimination mix for 5 min at 37 C, then place immediately on ice for at least 1 min. 4. Add 6 µl BC4 Solution to each well, mix by carefully pipetting up and down (can be done with a multi-channel pipettor). Centrifuge briefly to collect residual liquid from the sides of the tubes. 5. Program a thermal cycler for a single cycle as follows: 42 C for 60 min, 95 C for 5 min, 4 C hold. Place the 96-well plate in the cycler and run the program. This is the reverse transcription step. 6. Place the reactions on ice and proceed with the preamplification protocol. If you wish to store the reactions, transfer them to a 15 to 30 C freezer. Preamplification using RT 2 PreAMP Primer Mix Format H 7. Thaw RT 2 PreAMP Primer Mix and RT² PreAMP PCR Mastermix (PA- 30) on ice. Mix each solution by flicking the tubes. Centrifuge briefly to collect residual liquid from the sides of the tubes and then store on ice. 8. Prepare preamplification mix according to Table 10. Table 10. Preamplification mix Component Amount for one sample Amount for 96 wells* RT 2 PreAMP Primer Mix 3 µl 330 µl RT² PreAMP PCR Mastermix (PA-30) 5 µl 550 µl Total volume 8 µl 880 µl * These volumes provide 15% more mix than is required to allow for pipetting errors. 9. Pipet 8 µl preamplification mix into each well of an empty 96-well plate. 10. Add 2 µl of first-strand cdna from each well of the 96-well plate in step 6 to each well of the 96-well plate in step 9 using an 8-channel pipettor. The remaining first-strand cdna can be stored for use in future experiments. 11. Mix by carefully pipetting up and down and spin briefly. RT 2 Profiler PCR Array Handbook 12/

44 12. Program the real-time cycler according to Table 11. Place the 96-well plate in the real-time cycler and start the program. Table 11. Cycling conditions for preamplification Cycles Duration Temperature Comments 1 10 min 95 C HotStart DNA Taq Polymerase is activated by this heating step s 95 C 2 min 60 C Hold 4 C 13. When cycling is finished, take the plate from the real-time cycler and place on ice. 14. Add 1 µl Side Reaction Reducer to each well. Mix gently by pipetting up and down and spin briefly. 15. Incubate at 37 C for 15 min followed by heat inactivation at 95 C for 5 min. 16. Add 44 µl low EDTA TE buffer (0.1 mm EDTA) to each well. This is a 5-fold dilution (11 µl preamplification mix + 44 µl buffer). This dilution can be optimized if desired. (Undiluted cdna can be used for qpcr if needed.) 17. Place on ice prior to real-time PCR, or store at 15 to 30 C. Sample mix preparation 18. Prepare a sample mix according to Table RT 2 Profiler PCR Array Handbook 12/2014

45 Table 12. Sample mix Component Volume for one reaction Volume for a BioMark 96.96/48.48 Dynamic Array * 2x Microfluidics qpcr Master Mix 3 µl 330/165 µl 20x DNA Binding Dye Sample Loading Reagent (Fluidigm, cat. no ) 1x Low EDTA-TE buffer (0.1 mm EDTA) 0.3 µl 33/16.5 µl 0.7 µl 77/38.5 µl Total volume 4.0 µl 440/220 µl * These volumes provide 15% more mix than is required to allow for pipetting errors. 19. Pipette 53 µl (96.96 Dynamic Array) or 26 µl (48.48 Dynamic Array) sample mix into each tube of an 8-strip PCR tube. 20. Using an 8-channel pipettor, transfer 4 µl sample mix into each well of an empty 96-well plate (for the Dynamic Array, use only half of the 96-well plate). 21. Add 2 µl of each preamplified sample from step 17 to a well of the 96-well plate containing the sample mix. Note: Preamplified sample can be transferred using an 8-channel pipettor. 22. Cover the plate with plate sealer. Mix and spin briefly. 23. Label the plate as sample. Assay mix preparation 24. Remove the RT 2 Profiler PCR Array Format H from 15 to 30 C. Thaw for 10 min at room temperature (15 25 C). Briefly vortex and spin the plate to bring the contents to the bottom of the wells. 25. Mark the caps of the RT 2 Profiler PCR Array so that they can be replaced in the original order. Remove the caps. 26. Pipet 45 µl 2x Assay Loading Reagent (provided by Fluidigm) into each tube of an 8-strip PCR tube. 27. Transfer 3 µl 2x Assay Loading Reagent from the 8-strip tube into each well of an empty 96-well plate. This step can be performed using an 8-channel pipettor. RT 2 Profiler PCR Array Handbook 12/

46 Note: For a Dynamic Array, all 96 assays can be used at one time. When using a Dynamic Array, only 48 assays can be used at once. A second Dynamic Array must be run to utilize all 96 assays. 28. Transfer 3 µl from each well of the RT 2 Profiler PCR Array to the corresponding well of the 96-well plate from step Cover the plate with a plate sealer. Mix by vortexing and spin briefly. 30. Label this plate as assay. Priming and loading the Fluidigm BioMark HD Dynamic Array 31. Peel the blue protective film from the underside of the BioMark Chip. Place the BioMark Dynamic Array into the IFC Controller. 32. Prime the Dynamic Array using standard Fluidigm protocols. For details, consult the Fluidigm or Real-Time PCR Workflow Reference Guide. 33. Using an 8-channel pipettor, aliquot 5 µl from each well of the sample plate into appropriate sample inlets on the BioMark Dynamic Array (loading wells on the right side of the chip). 34. Using an 8-channel pipettor, aliquot 5 µl from each well of the assay plate into appropriate assay inlets on the BioMark Dynamic Array (loading wells on the left side of the chip). 35. Using the IFC Controller HX (96.96 Dynamic Arrays) or the IFC Controller MX (48.48 Dynamic Arrays), run the Load Mix (136x) Script for IFCs or the Load Mix (113x) Script for IFCs. 36. Remove the BioMark Dynamic Array from the IFC Controller. 37. Remove any dust particles from the BioMark Chip surface. Running the BioMark Dynamic Array IFC 38. Double-click the Data Collection Software icon to launch the software. 39. Click Start a New Run, place the chip into the reader, and click Load. 40. Verify chip barcode and chip type, choose project settings (if applicable), and click Next. 41. Chip run file: Select New or Predefined, browse to a file location for data storage, and click Next. 42. For Application, Reference, Probes, select the following: a) Application Type: Gene Expression, b) Passive Reference: ROX, c) Select Assay: single probe, d) Select probe type: EvaGreen. Click Next. 46 RT 2 Profiler PCR Array Handbook 12/2014

47 43. Click Browse to find thermal protocol file GE 96x96 Standard v1.pcl. or GE 48x48 Standard v1.pcl. Note: Make sure that you use a specific protocol or specific protocol depending on the Dynamic Array type. 44. Change the thermal protocol file to the conditions in Table 13. Thermal cycling protocols can be downloaded at Table 13. Cycling conditions for Fluidigm BioMark Dynamic Array IFCs Cycles Duration Temperature Comments s 1800 s 600 s 50 C 70 C 25 C Thermal Mix* (only for Dynamic Array IFC, Thermal Mix not needed for Dynamic Array IFC) s 95 C HotStart DNA Taq Polymerase is activated by this heating step s 94 C 60 s 60 C Perform fluorescence data collection. Ramp rate: Slow 1 C/s. * If you are using a Dynamic Array IFC, add a Thermal Mix segment by checking the box. The Thermal Mix is a step that helps the assay and sample chambers diffuse better on the small chambers on the Dynamic Array. You do not need a Thermal Mix if you are using any kind of chip other than the Dynamic Array IFC. 45. Confirm that Auto Exposure is selected and click Next. 46. Verify the Dynamic Array run information and click Start Run. RT 2 Profiler PCR Array Handbook 12/

48 Troubleshooting Guide This troubleshooting guide may be helpful in solving any problems that may arise. For more information, see also the Frequently Asked Questions page at our Technical Support Center: The scientists in QIAGEN Technical Services are always happy to answer any questions you may have about either the information and protocols in this handbook or sample and assay technologies (for contact information, see back cover or visit Comments and suggestions Presence of genomic DNA contamination a) DNase digestion not performed b) RT 2 First Strand Kit not used We strongly recommend performing the oncolumn DNase digestion step when purifying RNA using the RNeasy Mini Kit. We strongly recommend using the RT 2 First Strand Kit for cdna synthesis. This kit includes a genomic DNA elimination step. c) Reagents, tips, or tubes contaminated d) Genomic DNA difficult to remove See Preparing a workspace free of DNA contamination, page 22. If using the RT 2 RNA QC PCR Array, the no template control (NTC) indicates the level of DNA contamination in the experimental setup. Fold-changes in gene expression may still be obtained. However, it is very important to validate any results for individual genes by a separate more rigorous real-time PCR analysis that includes a minus RT control. Inefficient reverse transcription Poor quality RNA Check the A 260 :A 280 and A 260 :A 230 ratios of RNA samples. Be sure to perform the dilutions for spectrophotometry in RNase-free Tris ph 8.0. If necessary, repurify RNA using a spin-column method such as the RNeasy Mini Kit. 48 RT 2 Profiler PCR Array Handbook 12/2014

49 Poor PCR amplification efficiency a) Real-time cycler sensitivity Comments and suggestions Real-time cyclers vary in their level of sensitivity. From the positive PCR control (PPC), if an average C T PPC value of 20 ± 2 is difficult to obtain, the observed average C T PPC value should be acceptable as long as it does not vary by more than 2 cycles between RT 2 Profiler PCR Arrays. b) Cycling program incorrect Be sure that the initial heat activation step at 95 C was lengthened to 10 minutes from the shorter time in the default program. Be sure that all other cycle parameters also have been correctly entered according to the recommendations in the protocol. c) Poor quality RNA Check the A 260 :A 280 and A 260 :A 230 ratios of RNA samples. Be sure to perform the dilutions for spectrophotometry in RNase-free Tris ph 8.0. If necessary, repurify RNA using a spin-column method such as the RNeasy Mini Kit. RT 2 Profiler PCR Array Handbook 12/

50 Appendix A: Data Analysis Using the C T Method Visit our free PCR Array Data Analysis Web portal at At the PCR Array Data Analysis Web Portal, C T data can be entered and the Web-based software will automatically perform quantification using the C T method as described below and interpretation of the control wells. The PCR Array Data Analysis Web Portal presents results in a tabular format, a scatter plot, a three-dimensional profile, and a volcano plot (when replicates are included). Data analysis using the C T method for 96-well and 384- well formats Data analysis for formats A, C, D, E, F, G is described. For data analysis using format H with 96 x 96 microfluidic chips, visit A1. Change all C T values reported as greater than 35 or as N/A (not detected) to 35. At this point, any C T value equal to 35 is considered a negative call. A2. Examine the C T values of the genomic DNA control wells (GDC) as follows. Note: If the RT 2 PreAMP cdna Synthesis Kit was used for preamplification, consult the RT 2 PreAMP cdna Synthesis Handbook for the correct control values. Calculate C T GDC. If the value is greater than 35, the level of genomic DNA contamination is too low to affect gene expression profiling results. No action is needed. If the value is less than 35, genomic DNA contamination is evident. See the Troubleshooting Guide, page 48. A3. Examine the C T values of the reverse transcription control (RTC) using the values for the positive PCR control (PPC), as follows. Note: If RT 2 PreAMP cdna Synthesis Kit was used for preamplification, consult the RT 2 PreAMP cdna Synthesis Handbook for the correct control values. Calculate ΔC T = AVG C T RTC AVG C T PPC. If this value is less than 5, then no inhibition of the reversetranscription reaction is apparent. No action is needed. If this value is greater than 5, there is evidence of impurities that may have inhibited the reverse transcription reaction. See the Troubleshooting Guide, page RT 2 Profiler PCR Array Handbook 12/2014

51 A4. Examine the C T values of the positive PCR control wells (PPC) as follows. Calculate C T PPC. The average C T PPC value should be 20 ± 2 on each RT 2 Profiler PCR Array and should not vary by more than 2 cycles between RT 2 Profiler PCR Arrays being compared. Larger differences in average C T PPC values between samples indicate the presence of PCR amplification inhibitors. This means that the RNA samples require further purification. An average value of C T PPC that is consistently greater than 22 for all samples may indicate a problem with the cycling conditions or may simply be indicative of the relative sensitivity of your instrument. See the Troubleshooting Guide, page 48. A5. Calculate the C T for each pathway-focused gene in each plate using the C T values for the gene of interest (GOI) and the housekeeping genes used for normalization (HKG). Use the formula: C T = C T GOI C T AVG HKG Note: The expression level of the housekeeping genes chosen for normalization must not be influenced by the experimental conditions. If one or more such housekeeping genes have been previously identified by independent means and if the RT 2 Profiler PCR Array reproduces previous results, use the average of their C T values in the equation above. If an appropriate housekeeping gene has not been previously identified, use the average C T value of all housekeeping genes. Alternatively, use zero in the place of the average C T HKG for each group to be compared, and rely on the consistency in the quantity and quality of the original input total RNA to effectively normalize the results. A6. When biological and/or technical replicates are performed, calculate the average C T value of each gene (each well) across those replicate arrays for each treatment group. A7. Calculate the C T for each gene across 2 RT 2 Profiler PCR Arrays (or groups of samples). Use the formula: C T = C T (group 2) C T (group 1) where group 1 is the control sample or group of control samples and group 2 is the experimental sample or group of experimental samples. A8. Calculate the fold-change for each gene from group 1 to group 2 as 2 (- CT). Note: If the fold-change is greater than 1, the result may be reported as a fold upregulation. If the fold-change is less than 1, the negative inverse of the result may be reported as a fold downregulation. Fold-change ratio calculation will not be reliable when raw C T values from both groups are greater than 35. RT 2 Profiler PCR Array Handbook 12/

52 Note: The free online software GNCPro outlines gene and pathway interactions ( Data analysis using the C T method for Rotor-Disc formats A1. Change all C T values reported as greater than 33 or as N/A (not detected) to 33. At this point, any C T value equal to 33 is considered a negative call. A2. Examine the C T values of the genomic DNA control wells (GDC) as follows. Calculate C T GDC. If the value is greater than 33, the level of genomic DNA contamination is too low to affect gene expression profiling results. No action is needed. If the value is less than 33, genomic DNA contamination is evident. See the Troubleshooting Guide, page 48. A3. Examine the C T values of the reverse transcription control (RTC) using the values for the positive PCR control (PPC), as follows. Calculate ΔC T = AVG C T RTC AVG C T PPC. If this value is less than 5, then no inhibition of the reversetranscription reaction is apparent. No action is needed. If this value is greater than 5, there is evidence of impurities that may have inhibited the reverse transcription reaction. See the Troubleshooting Guide, page 48. A4. Examine the C T values of the positive PCR control wells (PPC) as follows. Calculate the C T PPC. The average C T PPC value should be 14 ± 2 on each RT 2 Profiler PCR Array and should not vary by more than 2 cycles between RT 2 Profiler PCR Arrays being compared. Larger differences in average C T PPC values between samples indicate the presence of PCR amplification inhibitors. This means that the RNA samples require further purification. An average value of C T PPC that is consistently greater than 16 for all samples may indicate a problem with the cycling conditions or may simply be indicative of the relative sensitivity of your instrument. See the Troubleshooting Guide, page RT 2 Profiler PCR Array Handbook 12/2014

53 A5. Calculate the C T for each pathway-focused gene in each Rotor-Disc using the C T values for the gene of interest (GOI) and the housekeeping genes used for normalization (HKG). Use the formula: C T = C T GOI C T AVG HKG Note: The expression level of the housekeeping genes chosen for normalization must not be influenced by the experimental conditions. If one or more such housekeeping genes have been previously identified by independent means and if the RT 2 Profiler PCR Array reproduces previous results, use the average of their C T values in the equation above. If an appropriate housekeeping gene has not been previously identified, use the average C T value of all housekeeping genes. Alternatively, use zero in the place of the average C T HKG for each group to be compared, and rely on the consistency in the quantity and quality of the original input total RNA to effectively normalize the results. A6. When biological and/or technical replicates are performed, calculate the average C T value of each gene (each well) across those replicate arrays for each treatment group. A7. Calculate the C T for each gene across 2 RT 2 Profiler PCR Arrays (or groups of samples). Use the formula: C T = C T (group 2) C T (group 1) where group 1 is the control sample or group of control samples and group 2 is the experimental sample or group of experimental samples. A8. Calculate the fold-change for each gene from group 1 to group 2 as 2 (- CT). Detailed mathematical explanation of C T data analysis method Due to the inverse proportional relationship between the threshold cycle (Ct) and the original gene expression level, and the doubling of the amount of product with every cycle, the original expression level (L) for each gene of interest is expressed as: L = 2 C T To normalize the expression level of a gene of interest (GOI) to a housekeeping gene (HKG), the expression levels of the two genes are divided: RT 2 Profiler PCR Array Handbook 12/

54 To determine fold change in gene expression, the normalized expression of the GOI in the experimental sample is divided by the normalized expression of the same GOI in the control sample: The complete calculation is as follows: 54 RT 2 Profiler PCR Array Handbook 12/2014

55 Appendix B: Protocol for Housekeeping Genes RT 2 Profiler PCR Arrays This protocol is for cdna synthesis and real-time PCR using Housekeeping Genes RT 2 Profiler PCR Arrays (cat. no PAHS-000, PAMM- 000, and PARN-000). Procedure cdna synthesis using the RT 2 First Strand Kit Perform a reverse-transcription reaction for each sample to be characterized on the array including one sample representing your biological or experimental control. Follow the protocol on page 27. Real-time PCR Follow the protocol on page 29, with the following changes to the preparation of the PCR components mix and dispensing of the PCR components mix into the Housekeeping Gene RT 2 Profiler PCR Array. 1. Prepare the PCR components mix in a 5 ml tube or a loading reservoir as described in Table 13. Table 13. PCR components mix Component 2x RT 2 SYBR Green Mastermix Volume for 96-well format Volume for 384-well format Volume for Rotor-Disc format µl 135 µl 270 µl cdna synthesis reaction 27 µl 12 µl 27 µl RNase-free water µl 123 µl 243 µl Total volume 675 µl 270 µl 540 µl Volume per well 25 µl 10 µl 20 µl 2. Dispense the PCR components mix into the RT 2 Profiler PCR Array. Note: Organize sample loading onto the arrays very carefully making sure to characterize each sample in duplicate and to include a replicate of the control sample on each plate. For example, up to 4 samples can be characterized in duplicate on a single array or duplicate determinations may be made on 2 separate arrays for larger numbers of samples. RT 2 Profiler PCR Array Handbook 12/

56 Samples Housekeeping genes A G1 G2 G3 G4 G5 G6 G7 G8 G9 G10 G11 G12 B G1 G2 G3 G4 G5 G6 G7 G8 G9 G10 G11 G12 C G1 G2 G3 G4 G5 G6 G7 G8 G9 G10 G11 G12 D G1 G2 G3 G4 G5 G6 G7 G8 G9 G10 G11 G12 E G1 G2 G3 G4 G5 G6 G7 G8 G9 G10 G11 G12 F G1 G2 G3 G4 G5 G6 G7 G8 G9 G10 G11 G12 G G1 G2 G3 G4 G5 G6 G7 G8 G9 G10 G11 G12 H G1 G2 G3 G4 G5 G6 G7 G8 G9 G10 G11 G12 Figure 7. Layout of the Housekeeping Genes RT 2 Profiler PCR Arrays in 96-well plates. Data analysis using the C T method 3. For each sample, average the duplicate determinations of the C T values from each sample for each housekeeping gene. 4. For each housekeeping gene, calculate the C T (the difference between the C T value of the gene in each experimental sample and the C T value of the gene in the control sample). 5. Choose the housekeeping genes with the smallest C T value across the samples of interest to normalize the results of future RT-PCR experiments for input total RNA loading. More than one housekeeping gene may be chosen for analyses. Simply monitor the expression of all of these housekeeping genes, and use their average C T value as the normalization factor for each sample. 56 RT 2 Profiler PCR Array Handbook 12/2014

57 References QIAGEN maintains a large, up-to-date online database of scientific publications utilizing QIAGEN products. Comprehensive search options allow you to find the articles you need, either by a simple keyword search or by specifying the application, research area, title, etc. For a complete list of references, visit the reference database online at or contact QIAGEN Technical Services or your local distributor. RT 2 Profiler PCR Array Handbook 12/

58 Ordering Information Product Contents Cat. no. RT² Profiler PCR Array Arrays of assays for disease, pathway, or functionally related genes; available in 96-well, 384-well, and Rotor-Disc 100 formats RT² RNA QC PCR Array Array for quality control analysis prior to experiments using RT² Profiler PCR Arrays; available in 96-well, 384-well, and Rotor-Disc 100 formats RT² First Strand Kit (12) RT 2 SYBR Green qpcr Mastermix (2)* RT 2 SYBR Green Fluor qpcr Mastermix (2)* RT 2 SYBR Green ROX qpcr Mastermix (2)* RT 2 SYBR Green ROX FAST Mastermix (2)* For 12 x 20 µl first strand cdna synthesis reactions; Buffer GE (30 µl), Buffer BC3 (60 µl), RE3 Reverse Transcriptase Mix (28 µl), Control P2 (18 µl), RNase-Free Water (1 ml) For 2 x 96 assays in 96-well plates; suitable for use with real-time cyclers that do not require a reference dye; 2 x 1.35 ml Mastermix For 2 x 96 assays in 96-well plates; suitable for use with real-time cyclers that use fluorescein reference dye; 2 x 1.35 ml Mastermix For 2 x 96 assays in 96-well plates; suitable for use with real-time cyclers that use ROX reference dye; 2 x 1.35 ml Mastermix For 2 x 96 assays in 96-well plates; suitable for use with real-time cyclers that use ROX reference dye, including the Rotor-Gene Q and Rotor-Gene 6000; 2 x 1.35 ml Mastermix * Larger kit sizes available; please inquire. 58 RT 2 Profiler PCR Array Handbook 12/2014

59 Product Contents Cat. no. Related products Human XpressRef Universal Total RNA Mouse XpressRef Universal Total RNA Rat XpressRef Universal Total RNA RT² PreAMP cdna Synthesis Kit (12) RT² PreAMP Pathway Primer Mix RT² Microfluidics qpcr Reagent System 2 tubes each containing 100 µg human RNA at 1 mg/ml 2 tubes each containing 100 µg mouse RNA at 1 mg/ml 2 tubes each containing 100 µg rat RNA at 1 mg/ml For 12 x 20 µl first-strand cdna synthesis reactions: Buffer GE, Buffer BC3, RE3 Reverse Transcriptase Mix, RNase Inhibitor, Control P2, RNase- Free Water; for 48 x 25 µl preamplification reactions: RT 2 PreAMP PCR Mastermix (600 µl); Side Reaction Reducer (96 µl) Pathway-focused primer mixes for use with the RT² PreAMP cdna Synthesis Kit For 96 x 20 µl first strand cdna synthesis reactions; 1 tube Buffer GE2 (750 µl/tube), 1 tube BC4 Reverse Transcriptase Mix (750 µl/tube); RT 2 PreAMP PCR Mastermix (600 µl); Side Reaction Reducer (96 µl); 2x Microfluidics EvaGreen qpcr Master Mix (1650 µl) mirneasy Mini Kit (50)* For 50 preps: 50 RNeasy Mini Spin Columns, Collection Tubes (1.5 ml and 2 ml), QIAzol Lysis Reagent, RNase- Free Reagents and Buffers RNase-Free DNase Set (50) For DNase digestion during RNA purification: 1500 units RNase-free DNase I, RNase-free Buffer RDD, and RNase-free water for 50 RNA minipreps * Larger kit sizes available; please inquire. RT 2 Profiler PCR Array Handbook 12/

60 Product Contents Cat. no. mirneasy Micro Kit (50) For 50 total RNA preps: 50 RNeasy MinElute Spin Columns, Collection Tubes (1.5 ml and 2 ml), QIAzol Lysis Reagent, RNase-Free Reagents and Buffers mirneasy FFPE Kit (50) PAXgene Blood RNA Kit (50) RNeasy Microarray Tissue Mini Kit (50) QIAamp RNA Blood Mini Kit (50) RT² PCR Array Loading Reservoir 384EZLoad Covers 50 RNeasy MinElute Spin Columns, Collection Tubes, Proteinase K, RNase- Free DNase I, DNase Booster Buffer, RNase-Free Buffers, RNase-Free Water 50 PAXgene Spin Columns, 50 PAXgene Shredder Spin Columns, Processing Tubes, RNase-Free DNase I, RNase-free reagents and buffers; To be used in conjunction with PAXgene Blood RNA Tubes RNeasy Mini Spin Columns, Collection Tubes, QIAzol Lysis Reagent, RNasefree reagents and buffers 50 QIAamp Mini Spin Columns, 50 QIAshredder Spin Columns, Collection Tubes (1.5 ml and 2 ml), RNase-free reagents and buffers 12 x 5 ml capacity, irradiation-sterilized loading reservoirs Pack of 4 color-coded covers for loading 384-well plates For up-to-date licensing information and product-specific disclaimers, see the respective QIAGEN kit handbook or user manual. QIAGEN kit handbooks and user manuals are available at or can be requested from QIAGEN Technical Services or your local distributor. 60 RT 2 Profiler PCR Array Handbook 12/2014

61 Notes RT 2 Profiler PCR Array Handbook 06/

62 Notes 62 RT 2 Profiler PCR Array Handbook 12/2014

63 Trademarks: QIAGEN, QIAamp, QIAzol, QIAgility, RNeasy, Rotor-Gene, Rotor-Disc (QIAGEN Group); Fluidigm, BioMark, Dynamic Array (Fluidigm Corp.); PAXgene (PreAnalytiX GmbH); Roche, LightCycler, TaqMan (Roche Group); Applied Biosystems, ROX, StepOnePlus, ViiA (Applera Corporation or its subsidiaries); Eppendorf, Mastercycler (Eppendorf AG); Stratagene, Mx3005P, Mx3000P, Mx4000 (Stratagene); Bio-Rad, icycler, Chromo4, CFX96, DNA Engine Opticon, CFX384, iq, MyiQ (Bio-Rad Laboratories, Inc.); Excel (Microsoft, Inc.); LabChip (Caliper Technologies Corp.); Agilent (Agilent Technologies, Inc.); FACS (Becton Dickinson and Company); SmartCycler (Cepheid); DNA-free (Ambion, Inc.); SYBR (Life Technologies Corporation); TRIzol, RNAzol (Molecular Research Center, Inc.); EvaGreen (Biotium, Inc.). Registered names, trademarks, etc. used in this document, even when not specifically marked as such, are not to be considered unprotected by law. Limited License Agreement Use of this product signifies the agreement of any purchaser or user of the RT 2 Profiler PCR Array to the following terms: 1. The RT 2 Profiler PCR Array may be used solely in accordance with the RT 2 Profiler PCR Array Handbook and for use with components contained in the Kit only. QIAGEN grants no license under any of its intellectual property to use or incorporate the enclosed components of this Kit with any components not included within this Kit except as described in the RT 2 Profiler PCR Array Handbook and additional protocols available at 2. Other than expressly stated licenses, QIAGEN makes no warranty that these Kits and/or their use(s) do not infringe the rights of third-parties. 3. These Kits and their components are licensed for one-time use and may not be reused, refurbished, or resold. 4. QIAGEN specifically disclaims any other licenses, expressed or implied other than those expressly stated. 5. The purchaser and user of these Kits agree not to take or permit anyone else to take any steps that could lead to or facilitate any acts prohibited above. QIAGEN may enforce the prohibitions of this Limited License Agreement in any Court, and shall recover all its investigative and Court costs, including attorney fees, in any action to enforce this Limited License Agreement or any of its intellectual property rights relating to these Kits and/or their components. For updated license terms, see LIMITED LICENSE STATEMENTS Use of this product is covered by one or more of the following US patents and corresponding patent claims outside the US: 5,994,056 and 6,171,785. The purchase of this product includes a limited, nontransferable immunity from suit under the foregoing patent claims for using only this amount of product for the purchaser's own internal research. No right under any other patent claim and no right to perform commercial services of any kind, including without limitation reporting the results of purchaser's activities for a fee or other commercial consideration, is conveyed expressly, by implication, or by estoppel. This product is for research use only. Diagnostic uses under Roche patents require a separate license from Roche. Further information on purchasing licenses may be obtained by contacting the Director of Licensing, Applied Biosystems, 850 Lincoln Centre Drive, Foster City, California 94404, USA. This product is provided under an agreement between Molecular Probes, Inc. and SABiosciences and the manufacture, use, sale, or import of this product is subject to one or more of U.S. Patent Nos. 5,436,134; 5,658,751 and corresponding international equivalents, owned by Invitrogen Corp. The purchase of this product conveys to the buyer the non-transferable right to use the purchased amount of the product and components of the product in research conducted by the buyer, where such research does not include testing, analysis or screening services for any third party in return for compensation on a per test basis. The buyer cannot sell or otherwise transfer (a) this product (b) its components or (c) materials made using this product or its components to a third party or otherwise use this product or its components or materials made using this product or its components for Commercial Purposes. Commercial Purposes means any activity by a party for consideration and may include, but is not limited to: (1) use of the product or its components in manufacturing; (2) use of the product or its components to provide a service, information, or data; (3) use of the product of its components for therapeutic, diagnostic or prophylactic purposes; or (4) resale of the product or its components, whether or not such product or its components are resold for use in research. For information on purchasing a license to this product for purposes other than research, contact Molecular Probes, Inc., Business Development, Willow Creek Road, Eugene, OR Tel: (541) , Fax: (541) The purchase of this product includes a limited, non-transferable license under specific claims of U.S. Patent Nos. 6,174,670, 6,569,627 and 5,871,908, owned by the University of Utah Research Foundation or Evotec Biosystems GmbH and licensed to Idaho Technology, Inc. and Roche Diagnostics GmbH, to use only the enclosed amount of product according to the specified protocols. No right is conveyed, expressly, by implication, or by estoppel, to use any instrument or system under any claim of U.S. Patent Nos. 6,174,670, 6,569,627 and 5,871,908, other than for the amount of product contained herein. The purchase of this product (products comprising ROX dye) includes a limited, non-transferable right to use the purchased amount of the product to perform Applied Biosystems patented Passive Reference Method for the purchaser s own internal research. No right under any other patent claim and no right to perform commercial services of any kind, including without limitation reporting the results of purchaser's activities for a fee or other commercial consideration, is conveyed expressly, by implication, or by estoppel. This product is for research use only. For information on obtaining additional rights, please contact outlicensing@lifetech.com or Out Licensing, Life Technologies, 5791 Van Allen Way, Carlsbad, California QIAGEN, all rights reserved. RT 2 Profiler PCR Array Handbook 06/

64 Australia Austria Belgium Brazil Canada China Denmark Finland France Germany Hong Kong India Ireland Italy Japan Korea (South) Luxembourg Mexico The Netherlands Norway Singapore Sweden Switzerland UK USA /2014 Sample & Assay Technologies